Species-specific multiplex PCR for the diagnosis of Brucella ovis, Actinobacillus seminis, and Histophilus somni infection in rams

Moustacas, Valéria Spyridion; Silva, Teane M. A.; Costa, Lourena E.; Xavier, Mariana N.; Junior, C.A. Carvalho; Costa, Érica Azevedo; Paixão, Tatiane Alves da; Santos, Renato L.

doi:10.1186/1746-6148-9-51

Cited by 23 publications

(23 citation statements)

References 21 publications

(46 reference statements)

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confidence: 99%

“…As shown in the results of analytical sensitivity tests, the detection limit of the multiplex PCR was lower than the singleplex PCR assays, when multiple parasites were simultaneously detected. This is expected, since in a multiplex PCR reaction for detection of multiple targets, all primer pairs will compete for limited reaction reagents, resulting in sub-optimal amplification efficiencies (Bilgiç et al 2013, Moustacas et al 2013.When applied to screening of the 104 field samples, the multiplex PCR and the 4 singleplex PCR methods were proven to be more effective for detection of the 4 target myxosporeans compared to microscopic examinations. During the microscopical detection, although the early stages of myxosporeans could be observed, only samples infected by mature spores were recorded as positive, as the early stages of myxo sporeans were difficult to distinguish morphologically to species level.…”

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Development of a multiplex PCR method for the simultaneous detection of four myxosporeans infecting gibel carp Carassius auratus gibelio

Li¹,

Zhai²,

Gu³

et al. 2017

Dis. Aquat. Org.

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Gibel carp Carassius auratus gibelio (Bloch), a commercially important freshwatercultured fish in China, is threatened by myxosporeans, particularly Thelohanellus wuhanensis, Myxobolus honghuensis, M. wulii and M. turpisrotundus. Here, we developed a multiplex PCR assay for simultaneous detection of these 4 myxosporeans. The specific primers for each species were designed based on the 28S rDNA gene of T. wuhanensis, the ITS-5.8S rDNA of M. honghuensis and M. wulii, and the 18S rDNA gene of M. turpisrotundus. Specificity testing confirmed that the 4 primer sets have no cross-reactivity with other related myxosporean species tested. Detection limits of the multiplex PCR assay were 0.2, 0.3, 3.1 and 3.8 spores for T. wuhanensis, M. honghuensis, M. wulii and M. turpisrotundus, respectively. Following screening of 104 field samples, the analytical sensitivity of the present multiplex PCR assay was found to be similar to the sensitivity obtained by the singleplex PCR assays and was higher than that of microscopic examination. Moreover, Kappa analysis showed a strong agreement between the results of the singleplex and multiplex PCR assays, indicating that the developed multiplex PCR assay was an efficient approach for the diagnosis of the 4 myxosporeans infecting gibel carp. KEY WORDS: Multiplex PCR · Molecular detection · Myxosporeans · Gibel carp · rDNA Resale or republication not permitted without written consent of the publisherDis Aquat Org 124: [31][32][33][34][35][36][37][38][39] 2017 forms plasmodia in the skin of the host and is responsible for chronic mortality and poor growth (Liu et al. 2014b). Minimizing the severe negative impact of myxosporidiosis on commercially important gibel carp is considered a priority in China. Early and accurate detection of myxosporeans could help fish farmers to carry out prompt drug therapy and minimize the likelihood of a myxo sporidiosis outbreak (Jia et al. 2015). Therefore, a simple and efficient assay for detection of myxo sporean pathogens is needed.Microscopic examination of squash preparations or histological sections is the most direct and commonly used method to detect and distinguish myxosporean parasites (St-Hilaire et al. 1997, Kelley et al. 2004). However, this approach can be time-and laborconsuming, and detection and identification is mainly based on the mature spore stages, with the early parasite stages likely to be neglected (Grabner et al. 2012, Mahony et al. 2015. Immunological methods based on antibodies or lectins (Knaus & El-Matbouli 2005, Estensoro et al. 2013) have also been developed. Nevertheless, these methods are generally restricted by cross-reactivity between different species (Lu et al. 2002, Estensoro et al. 2014, Jia et al. 2016. In recent years, PCR-based molecular detection and identification with higher sensitivity, specificity and rapidity has been utilised widely in myxo sporean examination (Qureshi et al. 2002, Cavender et al. 2004, Clark 2006, Grabner et al. 2012, Jeon et al. 2014. Given the multiple copies and moderate i...

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confidence: 99%

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confidence: 99%

Development of a multiplex PCR method for the simultaneous detection of four myxosporeans infecting gibel carp Carassius auratus gibelio

Li¹,

Zhai²,

Gu³

et al. 2017

Dis. Aquat. Org.

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“…The gold standard diagnosis of B. ovis infection is based on clinical examination, serology and semen bacteriology (Xavier et al, 2011;Poester et al, 2013), while for H. somni infections, only clinical examination and bacteriology are routinely performed. Semen and urine are the samples of choice for diagnosis (Xavier et al, 2010;Costa el al., 2012;Moustacas et al, 2013). These techniques are labor intensive and slow, whereas molecular techniques have been increasingly used, including conventional PCR (Xavier et al, 2010;Costa et al, 2012), nested PCR , and conventional multiplex PCR (Saunders et al, 2007;Moustacas et al, 2013).…”

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confidence: 99%

Real-time PCR for detection of Brucella ovis and Histophilus somni in ovine urine and semen

Moustacas

Silva

Costa

et al. 2015

Arq. Bras. Med. Vet. Zootec.

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“…Sheep epididymitis has been mainly associated with Brucella ovis and Actinobacillus seminis infections (Burgess 1982, Moustacas et al 2013. The pathogenesis of the disease caused by A. seminis has been explored to a small extent; the presence of pathogenicity factors in A. seminis, such as adhesins (Healey et al 1991) or RTX toxins (Schaller et al 2000), is likely to contribute to the development of the pathology.…”

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confidence: 99%

Distribution of lymphocytes, immunoglobulin-containing cells, macrophages, and dendritic cells in the accessory sex glands of rams experimentally infected with Actinobacillus seminis

et al. 2016

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The distribution of cells involved in the immune response in accessory sex glands of rams experimentally infected with Actinobacillus seminis was studied. Twelve one-year old rams were experimentally infected by intraurethral (IU) (n=4) and intraepididymal (IE) (n=4) route, and four control (CON) animals were used. The animals were slaughtered 35 days post-inoculation, samples were taken from accessory sex glands, and bacteriology and histopathology tests were performed. The presence of CD4, CD8 and TCRγδ (WC1) lymphocytes, CD45RO cells, macrophages (CD14), dendritic cells (CD1b), IgA-, IgG-and IgM-containing cells (IgCC) was determined. Animals of the IE group developed clinical epididymitis. No lesions were seen in rams of the IU group; two of the intraepididymal inoculated CON developed small lesions in the epididymis. A. seminis isolates were achieved from 6:16 (37.5%) accessory sex glands in the IE group, but not in the IU and CON groups. In the CON group, IgA-and IgM-containing cells predominated in the bulbourethral glands and the disseminated prostate, and they were scarce or null in the vesicles and ampullae. A significant increase of IgA-, IgG-and IgM-containing cells was confirmed in the seminal vesicles, the ampullae and the bulbourethral glands in the IE group. In the IE and IU groups, an increase in CD4, CD8, WC1, CD45RO and CD14 was evidenced in the vesicles and ampullae. CD1b dendritic cells were present in the ampullae and vesicles with inflammatory processes. A. seminis triggered a local immune response in the IE and IU groups. These results indicate a different pattern of infiltrating immune cells in the accessory sex glands of infected A. seminis rams.

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Species-specific multiplex PCR for the diagnosis of Brucella ovis, Actinobacillus seminis, and Histophilus somni infection in rams

Cited by 23 publications

References 21 publications

Development of a multiplex PCR method for the simultaneous detection of four myxosporeans infecting gibel carp Carassius auratus gibelio

Development of a multiplex PCR method for the simultaneous detection of four myxosporeans infecting gibel carp Carassius auratus gibelio

Real-time PCR for detection of Brucella ovis and Histophilus somni in ovine urine and semen

Distribution of lymphocytes, immunoglobulin-containing cells, macrophages, and dendritic cells in the accessory sex glands of rams experimentally infected with Actinobacillus seminis

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